Saccharopolyspora culture

Abstract

A process for preparing the antibiotic U-59,760. The process is a microbiological process using a biologically pure culture of the novel microbe Saccharopolyspora hirsuta strain 367, NRRL 12045. The antibiotic produced by the process is active against various microorganisms, for example, Staphylococcus aureus, Streptococcus pyogenes, and Klebsiella pneumoniae. Thus, antibiotic U-59,760 can be used in various environments to eradicate or control such bacteria.

Description

BRIEF SUMMARY OF THE INVENTION

The process of the invention utilizes the biologically pure culture of the novel microbe Saccharopolyspora hirsuta strain 367, NRRL 12045, to produce the useful antibiotic U-59,760. The physical and chemical characteristics of this antibiotic cannot be distinguished from the antibiotic known as compound 47444 which is disclosed in U.S. Pat. No. 4,148,883. The production of the antibiotic in U.S. Pat. No. 4,148,883 is accomplished by an entirely different microbe which is classified as a Nocardia.

DETAILED DESCRIPTION OF THE INVENTION

The microorganism used for the production of antibiotic U-59,760, as described herein, is a biologically pure culture of Saccharopolyspora hirsuta strain 367, NRRL 12045.

A subculture of this microorganism can be obtained from the permanent collection of the Northern Regional Research Laboratory, U.S. Department of Agriculture, Peoria, Ill., U.S.A. Its accession number in this depository is NRRL 12045. It should be understood that the availability of the culture does not constitute a license to practice the subject invention in derogation of patent rights granted with the subject instrument by governmental action.

The microorganism of this invention was studied and characterized by Alma Dietz and Grace P. Li of The Upjohn Company Research Laboratories.

An actinomycete isolated in the Upjohn soils screening laboratory has been characterized and found to have the macroscopic, microscopic and whole cell hydrolysate properties of the genus Saccharopolyspora [Iwasaki, A., N. Itoh, and T. Mori, 1979. A new broad-spectrum aminoglycoside antibiotic complex, sporaricin. II. Taxonomic studies on the sporaricin producing strain Saccharopolyspora hirsuta subsp. kobensis nov. subsp. J. Antibiotics. 32: 180-186.] [Lacey, J. and M. Goodfellow. 1975. A novel actinomycete from sugar-cane bagasse: Saccharopolyspora hirsuta gen. et sp. novl. J. Gen. Microbiol. 88: 75-87]. A comparison with the type culture Saccharopolyspora hirsuta ATCC 27875 is given in Tables 1 and 2. A comparison with the type culture and with the subspecies, Saccharopolyspora hirsuta ss. kobensis ATCC 20501 [Iwasaki, A. supra] based on data published for these strains is given in Table 3.

Unique properties of the genus Saccharopolyspora are its butyrous or gelatinous-type vegetative growth, sparse aerial growth which is best studied after 21 days incubation, yellow to orange to orange-tan vegetative growth and pigment production, spore chains developing in a sheath with unique hair tufts with truncated bases and smooth areas between the tufts, the presence of meso-diaminopimelic acid, arabinose and galactose in whole cell hydrolysates and in cell wall preparations. L-diaminopimelic acid was detected in addition to meso-DAP in our cell wall preparations.

No antibiotic production has been reported for the type culture; the subspecies kobensis produces the antibiotic complex sporaricin (KA-6606) [Iwasaki, A. supra]. The new isolate is distinguished by the production of antibiotic U-59,760 and U-59,761. The only significant difference among the strains is in their antibiotic production capability. Therefore, the new strain is designated Saccharopolyspora hirsuta strain 367.

The taxonomic methods used herein were those cited in Dietz [Dietz, A. 1954. Ektachrome transparencies as aids in actinomycete classification. Ann N.Y. Acad. Sci. 60: 152-154.] [Dietz, A. 1967. Streptomyces steffisburgensis sp. n. J. Bacteriol. 94: 2022-2026.], Dietz and Mathews [Dietz, A., and J. Mathews. 1971. Classification of Streptomyces spore surfaces into five groups. Appl. Microbiol. 21: 527-533.], Becker et al. [Becker, B., M. P. Lechevalier, and H. A. Lechevalier. 1966. Chemical composition of cell wall preparations from strains of various form-genera of aerobic actinomycetes. Appl. Microbiol. 13 236-243.], Lechevalier and Lechevalier [Lechevalier, H. A., and M. P. Lechevalier. 1970. A critical evaluation of the genera of aerobic actinomycetes, p. 393-405. In H. Prauser (ed.), The Actinomycetales. Gustav Fisher, Jena.] [Lechevalier, M. P., and H. A. Lechevalier. 1970. Chemical composition as a criterion in the classification of aerobic actinomycetes. Int. J. Syst. Bacteriol. 20: 435-443.], and Shirling and Gottlieb [Shirling, E. B., and D. Gottlieb. 1966. Methods for characterization of Streptomyces species. Int. J. Syst. Bacteriol. 16: 313-340.].

Color characteristics: Aerial mycelium gray to gray-pink (very sparse at 14 days). Melanin negative. Appearance on Ektachrome is given in Table 1. Surface colors of the vegetative growth were determined to be red (R) or yellow (Y) by matching the color with the chips in the Tresner and Backus [Tresner, H. D., and E. J. Backus. 1963. System of color wheels for streptomycete taxonomy. Appl. Microbiol. 11: 335-338.] color wheels.

Microscopic characteristics: Spore masses and spore chains, intact and fragmented, and flexuous or loosely spiraled chains, as observed by Scanning Electron Microscopy, appear to develop in a sheath which is at first almost smooth; then unique tufts of hairs (triangular at the base) are formed. The surface between the tufts is smooth. Finally, the sheath becomes covered with fine long hairs. The long sheaths are tangled and appear to arise from, or fuse to form pseudosporangia. As the chains come in contact with the substrate the spores become smooth in outline with a depressed or ridged appearance. "Empty" hyphae are noted in the developed chains. Microscopic characteristics are best noted after 21 days incubation at 28.degree.-37.degree. C. Nocardioform fragmentation may be seen in 21 day cultures.

Growth on carbon compounds: Under the test conditions of Shirling and Gottlieb [supra] growth was good on the postive control (basal medium plus D-glucose), sucrose, D-mannitol, D-fructose and raffinose. Growth was doubtful on L-arabinose and D-xylose. There was no growth on the negative control (basal medium only), inositol, rhamnose, and cellulose.

Whole cell analysis: meso-Diaminopimelic acid, arabinose and galactose were detected.

Cell wall analysis: meso-Diaminopimelic acid, L-diaminopimelic acid, arabinose and galactose were found.

Cultural and biochemical characteristics: See Table 2.

Temperature: There was no to very poor growth at 18.degree. C. on Bennett's and maltose-tryptone agars and poor growth on Czapek's sucrose agar. Growth was good at 24.degree.-45.degree. C. There was no growth at 55.degree. C.

TABLE 1__________________________________________________________________________Color characteristics* of Saccharopolyspora hirsuta ATCC 27875 andS. hirsuta strain 367 on Ektachrome S. hirsuta ATCC 27875 S. hirsuta strain 367Agar Medium Determination Chip Color Chip Color__________________________________________________________________________Bennett's S 71 moderate orange yellow 71 moderate orange yellow R 71 moderate orange yellow 71 moderate orange yellowCzapek's sucrose S 74 strong yellowish brown 67 brilliant orange yellow R 72 dark orange yellow 67 brilliant orange yellowMaltose-tryptone S 71 moderate orange yellow 71 moderate orange yellow R 71 moderate orange yellow 71 moderate orange yellowPeptone-iron S 68 strong orange yellow 68 strong orange yellow R 68 strong orange yellow 68 strong orange yellow0.1% Tyrosine S 73 pale orange yellow 71 moderate orange yellow R 73 pale orange yellow 71 moderate orange yellowCasein S 73 pale orange yellow 70 light orange yellow R 73 pale orange yellow 73 pale orange yellow__________________________________________________________________________ *Color was determined by comparison with NBS color chips (SP 440. Color: Universal Language and Dictionary of Names. U.S. Government Printing Office, Washington, DC 20402. SRM 2106. ISCCNBS Centroid Color Charts. Office of Standard Reference Material, Room B311, Chem. Building, Nationa Bureau of Standards, Washington, DC 20234. S = Surface R = Reverse TABLE 2__________________________________________________________________________Cultural and biochemical characteristics of Saccharopolyspora hirsutastrains.Agar medium Determination S. hirsuta ATCC 27875 S. hirsuta strain 367__________________________________________________________________________Peptone-iron S Colorless (V) Colorless or light tan wrinkled (V) R Pale yellow Orange-tan P -- Pale tan to orange-tan O Melanin negative Melanin negativeCalcium malate S Trace white (A) Trace gray (A) R Cream Pale gray cream P -- -- O Malate solubilized Malate slightly solubilizedGlucose asparagine S Colorless to light tan (V) Light tan (V) R Orange Orange-tan P Orange Orange-tanSkim milk S Tan (V) Orange-brown (V) R Orange-tan Dark orange-tan P Orange-tan Deep orange-tan O Casein solubilized Casein solubilizedTyrosine S Tan (V) Orange-tan (V) R Orange Orange P Orange Orange O Tyrosine solubilized Tyrosine solubilizedXanthine S Colorless (V) Pale tan (V) R Pale yellow Pale tan P Pale yellow Pale tan-peach O Xanthine solubilized Xanthine solubilized around growthNutrient starch S Colorless (V) Pale tan (V) R Pale yellow Pale tan P Very pale yellow Very pale tan O Starch hydrolyzed Starch hydrolyzedYeast extract-malt S Colorless (V) Pale tan (V)extract R Orange Pale-orange-tan P Orange OrangePeptone-yeast S Colorless (V) with very Colorless (V)extract-iron slight trace white (A)(ISP-6) R Yellow-tan Light orange-tan to tan O Melanin negative Melanin negativeTyrosine (ISP-7) S Trace white (A) Very pale orange (V) R Yellow tan Very pale orange O Melanin negative Melanin negativeGelatinPlain S Trace white (A) on Colorless to pale yellow (V) colorless surface pellicle P None None to trace pale yellow O Gelatin liquefied Gelatin liquefiedNutrient S Trace white (A) on Trace colorless (V) to trace yellow (V) pellicle white (A) on (V) P None None O Gelatin liquefied Gelatin liquefiedBrothSynthetic nitrate S No surface growth Trace white (A) on colorless (V) P None None O Compact bottom growth Compact to flocculent bottom No reduction growth No reductionNutrient nitrate S Trace white (A) on color- Trace white (A) on colorless less surface pellicle surface ring P None None O Flocculent bottom growth; Poor colorless compact bottom No reduction growth; No reductionLitmus milk S Pale gray (A) on yellow- Blue-gray surface ring tan surface ring P None Deep red-tan O Litmus not reduced Peptonization pH 6.7-7.3 pH 7.6-7.8__________________________________________________________________________ S = Surface O = Other characteristics R = Reverse (V) = Vegetative Growth P = Pigment (A) = Aerial growth TABLE 3__________________________________________________________________________Comparision of Saccharopolyspora hirsuta strainsTests S. hirsuta strain 367 S. hirsuta ATCC 27875 S. hirsuta kobense ATCC__________________________________________________________________________ 20501Physiological PropertiesTemperature Growth from 18-45C Growth from 25-45C Growth from 18-45COptimum Temperature 28-45C 37-40C 37-42CGelatin liquefaction Complete Positive at 27C Positive at 27CStarch hydrolysis Positive Positive PositiveAction on milk No coagulation No coagulation No coagulation Peptonization Peptonization PeptonizationMelanoid pigment Negative Negative NegativeproductionNitrate reduction Negative Negative PositiveCarbon Source UtilizationL-Arabinose .+-. - -D-Xylose .+-. + -L-Rhamnose - + -D-Glucose + + +D-Fructose ++ + +Sucrose + + +Raffinose ++ + +Inositol - + -D-Mannitol ++ + +__________________________________________________________________________

The compound of the invention process is produced when the elaborating organism is grown in an aqueous nutrient medium under submerged aerobic conditions. It is to be understood, also, that for the preparation of limited amounts surface cultures and bottles can be employed. The organism is grown in a nutrient medium containing a carbon source, for example, an assimilable carbohydrate, and a nitrogen source, for example, an assimilable nitrogen compound or proteinaceous material. Preferred carbon sources include glucose, brown sugar, sucrose, glycerol, starch, cornstarch, lactose, dextrin, molasses, and the like. Preferred nitrogen sources include cornsteep liquor, yeast, autolyzed brewer's yeast with milk solids, soybean meal, cottonseed meal, cornmeal, milk solids, pancreatic digest of casein, fish meal, distillers' solids, animal peptone liquors, meat and bone scraps, and the like. Combinations of these carbon and nitrogen sources can be used advantageously. Trace metals, for example, zinc, magnesium, manganese, cobalt, iron, and the like, need not be added to the fermentation media since tap water and unpurified ingredients are used as components of the medium prior to sterilization of the medium.

Production of the compound by the invention process can be effected at any temperature conducive to satisfactory growth of the microorganism, for example, between about 18.degree. and 40.degree. C., and preferably between about 20.degree. and 28.degree. C. Ordinarily, optimum production of the compound is obtained in about 3 to 15 days. The final pH of the fermentation is dependent, in part, on the buffers present, if any, and in part on the initial pH of the culture medium.

When growth is carried out in large vessels and tanks, it is preferable to use the vegetative form, rather than the spore form, of the microorganism for inoculation to avoid a pronounced lag in the production of the compound and the attendant inefficient utilization of the equipment. Accordingly, it is desirable to produce a vegetative inoculum in a nutrient broth culture by inoculating this broth culture with an aliquot from a soil, liquid N.sub.2 agar plug, or a slant culture. When a young, active vegetative inoculum has thus been secured, it is transferred aseptically to large vessels or tanks. The medium in which the vegetative inoculum is produced can be the same as, or different from, that utilized for the production of the compound, so long as a good growth of the microorganism is obtained.

A variety of procedures can be employed in the isolation and purification of the compound produced by the subject invention from fermentation beers. Isolation can be accomplished by extraction with solvents such as methylene chloride, acetone, butanol, ethyl acetate and the like; and silica gel chromatography can be used to purify crude preparations of the antibiotic.

In a preferred recovery process, the compound produced by the subject process is recovered from the culture medium by separation of mycelia and undissolved solids by conventional means, such as by filtration or centrifugation, and solvent extraction of both mycelial cake or clarified broth. The clarified broth can be extracted with a suitable solvent, for example, methylene chloride (preferred), ethylacetate, butanol, and MIBK. The extract can be evaporated under reduced pressure to a concentrate and the antibiotic recovered from this concentrate by subjecting the concentrate to chromatography over silica gel and eluting with methanol and methylene chloride.

The following examples are illustrative of the process of the invention, but are not to be construed as limiting. All percentages are by weight and all solvent mixture proportions are by volume unless otherwise noted.

EXAMPLE 1

Part A. Fermentation

A biologically pure culture Saccharopolyspora hirsuta strain 367, NRRL 12045, is used to inoculate 500-ml Erlenmeyer seed flasks containing 100 ml of sterile medium consisting of the following ingredients:

______________________________________Glucose monohydrate 25 g/lPharmamedia* 25 g/lTap water q.s. 1 liter______________________________________ *Pharmamedia is an industrial grade of cottonseed flour produced by Traders Oil Mill Company, Fort Worth, Texas.

The seed medium presterilization pH is 7.2. The seed inoculum is grown for three days at 28.degree. C. on a Gump rotary shaker operating at 250 rpm and having a 21/2 inch stroke.

After three days incubation, the seed medium is used to inoculate (the inoculation rate is 5 ml of seed inoculum per 100 ml of fermentation medium) a series of 500-ml Erlenmeyer flasks containing sterile fermentation medium consisting of the following ingredients:

______________________________________Glucose monohydrate 10 g/lDextrin 20 g/1Corn steep liquor 2.5 g/lNH.sub.4 NO.sub.3 3.0 g/lNaCl 2.0 g/lCaCO.sub.3 5.0 g/lph-7.2 (presterilization)______________________________________

The fermentation flasks are incubated at a temperature of 28.degree. C. on a Gump torary shaker operating at 250 rpm nd having a 21/2 inch stroke. Harvest is usually after about 5 days of fermentation. A typical 5 day fermentation has the following titers of antibiotic in the fermentation broth:

______________________________________Day S. lutea Assay, Bu/ml______________________________________2 8.03 10.44 10.45 11.2______________________________________

In the assay results, a biounit (BU) is defined as the concentration of the antibiotic which gives a 20 mm zone of inhibition under the standard assay condition. Thus, if, for example, a fermentation beer has to be diluted 1/100 to give a 20 mm zone of inhibition, the potency of such beer is 100 Bu/ml.

B. Recovery and Purification

The whole beer (ca. 5,000 l) from a fermentation, as described above, is adjusted to pH 7.3 with NaOH and filtered on a 30 inch filter press using diatomaceous earth as a filter aid. During the filtration operation wash water is applied to the filter cake. From the filtration operation is recovered 5,500 l of clear fermentation broth which is then extracted twice with methylene chloride (1,400 l each time) to give a total of 2.800 l of solvent extract. This solvent extract is concentrated in vacuo to 10 l. Assay on a standard S. lutea disc plate assay gives a value of 2424 Bu/ml.

The extract concentrate described above (9 l), is chromatographed over a column containing 9 kg of silica gel (E. Merck-silica gel 7734). The column is eluted as follows:

20 liters methylene chloride; then 40 liters 2% methanol in methylene chloride; then 150 liters 5% methanol in methylene chloride; then 100 liters 10% methanol in methylene chloride. Four liter fractions are collected after an 80 liter forerun. Fractions 5-8 contain antibiotic U-59,760 having the following characteristics:

Elemental Analysis: C, 64.95, H, 7.42, N, 2.49

Molecular Weight: 515.2482 (Mass spectroscopy) (C.sub.28 H.sub.37 NO.sub.8).

Optical Rotation: [a].sub.D.sup.25 +53.degree. (C, 0.0848 MeOH).

Solubilities: Soluble in methanol, ethanol and methylene chloride, and relatively insoluble in petroleum ether and cyclohexane.

Infrared Absorption Spectrum: Antibiotic U-59,670 has a characteristic infrared absorption spectrum in a mineral oil mull. Peaks are observed at the following wave lengths expressed in reciprocal centimeters.

______________________________________Band Frequency(Wave Numbers) Intensity______________________________________3459 S3330 S, sh.3139 M, sh.3025 M2957 S2922 S2855 S2725 W1725 S, sh.1704 S1688 S1554 M1455 S1411 S1377 S1354 S1339 S1315 S, sh.1307 S1276 S1265 S, sh.1240 S1205 M1169 S1109 S1082 S1060 S1045 S1031 S1010 S968 S956 S949 S937 M909 M882 M870 M, sh.857 M835 M794 M764 S747 S719 M699 M677 M638 M______________________________________ Key: S = Strong, M = Medium, W =0 Weak, sh. = shoulder ______________________________________Antimicrobial spectrum: InhibitionOrganism Zone Size (mm).sup.1______________________________________B. subtilis UC 564 0B. subtilis UC 6033 16S. aureus UC 70 36S aureus UC 3665 42S. aureus UC 6029 38S. lutea UC 130 42S. lutea UC 3383 41S. lutea sens 45K. pneumoniae UC 58 32E. coli UC 51 0S. schottmuelleri UC 126 0P. vulgaris UC 93 0P. aeruginosa UC 95 0M. avium UC 159 30P. oxalicum UC 1268 0S. pastorianus UC 1342 0R. sphaeroides UC 3238 21S. pyogenes UC 6055 16B. fragilis UC 6513 37C. perfringens UC 6509 48______________________________________

"UC" is a registered trademark of The Upjohn Company culture collection. These cultures can be obtained from The Upjohn Company in Kalamazoo, Mich., upon request.

Since antibiotic U-59,760 is active against S. aureus, it can be used to disinfect washed and stacked food utensils contaminated with this bacteria. Also, it can be used as a disinfectant on various dental and medical equipment contaminated with S. aureus. Further, antibiotic U-59,760 can be used as a bacteriostatic rinse for laundered clothes, and for impregnating papers and fabrics; and, it is also useful for suppressing the growth of sensitive organisms in plate assays, and other microbiological media.

Claims

1. A biologically pure culture of the microorganism Saccharopolyspora hirsuta strain 367, having the identifying characteristics of NRRL 12045, said culture being capable of producing the antibiotic U-59,760 in a recoverable quantity upon fermentation in an aqueous nutrient medium containing assimilable sources of carbon, nitrogen and inorganic substances.